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Macroendocytosis and endosome processing in snake motor boutons

机译:蛇运动钮扣中的大内吞和内体加工

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摘要

We have examined the processing of endosomes formed by macroendocytosis (ME), or bulk membrane retrieval, in active motor terminal boutons at the snake nerve–muscle synapse. Endocytic probes were imaged at light (FM1–43) and electron (horseradish peroxidase (HRP)) levels over stimulus frequencies representing low, intermediate and high levels of use. Endosomes formed rapidly (1–2 s) at all frequencies, concomitant with clathrin-mediated vesicular endocytosis (CME). Endosomes dissipated rapidly into vesicles (∼10 s). The dissipation rate was not influenced by activity. Many endosomes split into clusters of 2–20 smaller endosomes of varying size. Vesicles budded from these smaller endosomes, from large endosomes that had not undergone fission into smaller ones, and from precursor membrane infoldings that had not yet internalized. In snake, exocytosed vesicular membrane is not competent for reuse until after a delay (> 3 min). We found that time required for endosome processing is not responsible for this delay. Endosome processing might, however, limit availability of some vesicles for release at very high levels of use. Generally, endosome processing paralleled that of vesicles internalized directly from the plasma membrane via CME, regardless of stimulus frequency. There was no evidence for differential recruitment of ME versus CME depending upon level of use.
机译:我们已经检查了在蛇神经-肌肉突触的活动性运动终末反弹中,由巨噬细胞(ME)或体膜回收形成的内体的加工过程。内吞探针在代表低,中和高使用水平的刺激频率下以光(FM1-43)和电子(辣根过氧化物酶(HRP))水平成像。内体在所有频率下迅速形成(1-2秒),并伴有网格蛋白介导的囊泡内吞作用(CME)。内体迅速消散到囊泡中(约10 s)。耗散率不受活动的影响。许多内体分裂成2-20个大小不同的较小内体的簇。囊泡从这些较小的内体,尚未经历裂变的较大内体,以及尚未内在化的前体膜折叠中萌芽。在蛇中,胞浆囊泡膜不能再使用,直到延迟(> 3分钟)。我们发现内体加工所需的时间对此延迟不负责。然而,内体加工可能会限制某些囊泡的可用性,这些囊泡在非常高的使用水平下释放。通常,不管刺激频率如何,内体加工与直接通过CME从质膜内化的囊泡的加工平行。没有证据表明ME与CME会因使用水平的不同而不同。

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